一个水稻高效表达启动子Os252的分离

植物基因的表达受启动子的控制,高效表达启动子的分离及功能分析不仅是植物基因工程研究的重要研究方面,也是表达调控研究的重要内容。根据EST数据克隆了一个预测在水稻茎中高效表达的启动子Os252。将该启动子与GUS基因构建成表达载体并转入水稻。转基因水稻PCR分析表明,GUS基因已经成功地整合进水稻基因组中。GUS组织化学分析表明,Os252能启动GUS基因在水稻叶、茎以及胚乳中表达。进一步GUS酶活性的测定表明,叶和胚乳中Os252启动子活性分别是35S启动子的1.9和2.5倍。由于Os252来自于水稻,在叶和胚乳中活性高于35S启动子,因此该启动子可望用于水稻基因工程研究。     

水稻谷蛋白基因GluC启动子的克隆及表达分析

水稻谷蛋白仅在水稻种子胚乳中表达,其启动子是分离胚乳特异性表达启动子的理想材料。本研究克隆了GluC基因启动子pGluC,生物信息学分析表明pGluC内部含有胚乳特异性表达所需要的Skn-1 motif和ACGT-box元件。将pGluC启动子和7个5'端缺失启动子片段构建到pGPTV-GUS载体上,转化水稻愈伤组织,进行组织化学染色和GUS酶活分析。结果表明：全长及截短的-1 911、-1 611、-1 311 bp启动子均能驱动GUS基因在水稻种子胚乳中高效稳定表达。-999、-451、-203、-102 bp启动子失去了胚乳表达特异性,在根、茎或者叶中也检测到GUS表达。该结果为实现外源目的基因在水稻胚乳中特异高效表达提供了理论依据。     

水稻 ADP-葡萄糖焦磷酸化酶小亚基 I 基因的启动子分析

水稻（Oryce sativa L．）基因组中的ADP-葡萄糖焦磷酸化酶小亚基（ADP-Glucose pyrophosphorylase small subunit,OsAgpS）由两个基因编码,即OsAgpSl和OsAgpS2。其中OsAgpSl基因产生两个转录本OsAgpSla和OsAgpSlb,区别在第一个外显子的位置不同。通过RT—PCR方法分析了两个转录本在水稻组织和胚乳不同发育时期的表达特性;同时通过报告基因GUS检测了两个转录本上游转录调节区DNA片段的转录启动特性。结果表明,两个启动子与其下游转录本的表达模式完全一致,即OsAgpSla转录本和OsAgpSla上游启动子控制的GUS基因主要在胚乳中高水平表达,在叶片中有很低水平的表达;而OsAgpSlb转录本和OsAgpSlb上游启动子控制的GUS基因主要在叶片和胚乳发育早期低水平表达。这说明OsAgpSl基因产生的两个转录本是由不同的启动子控制转录的,OsAgpSla上游启动子可以作为胚乳表达用启动子。     

水稻OsWTF1基因启动子的克隆与表达分析

目的：分析水稻OsWTF1基因启动子的功能及核心序列。方法：利用PCR技术从水稻日本晴基因组中克隆了转录因子WTF1编码区5上游大小为2049bp的调控区域,命名为OsWTF1,将它和长度为1631、608、474、415bp的5端缺失体分别与GUS基因融合构建表达载体,并用农杆菌介导法转化水稻。结果：GUS组织化学分析表明,OsWTF1、Os1631能够驱动GUS基因在根、茎、叶、叶鞘、花药、颖壳上的表达,Os608,Os474,Os415能驱动GUS在根、茎、花药、颖壳中表达,在叶鞘中未表达,而且在叶中的表达也很微弱。结论：OsWTF1启动子核心序列可能位于-1bp--415bp之间,在-608bp--1631bp之间可能存在与基因叶肉特异表达相关的重要元件。     

参与水稻光合作用的PsbR3基因启动子的功能分析

本实验旨在研究水稻光合作用蛋白中各基因的表达模式. 采用RT-PCR和定量real-time PCR数据分析水稻不同组织的mRNA表达水平.结果显示,PsaK和PsbR3基因仅在茎、叶等绿色组织表达,而胚、胚乳部分均不表达.通过其启动子克隆、植物表达载体构建,以及农杆菌介导转化后,GUS组织染化分析和GUS荧光定量分析表明,两启动子均为组织特异性优势表达,PsbR3启动报告酶GUS在叶片中的表达活性为Actin启动子的3.29倍,而PsaK启动报告酶GUS在叶片中的表达活性低于Actin启动子的.这些初步结果提示,PsbR3启动子决定水稻绿色组织茎叶的优势表达,PsbR3基因可能参与水稻光合作用.     

水稻CesA4基因启动子与GUS基因融合表达

目的:利用GUS报告基因,研究水稻CesA4基因在水稻组织和器官的定位.方法:克隆水稻的CesA4基因的启动子并用GUS组织化学染色检测启动子与GUS基因融合表达情况.结果:成功克隆了水稻的CesA4基因的启动子,并发现水稻的CesA4基因在水稻的根、茎、叶、鞘、穗的纤维均有表达.结论:通过将水稻CesA4基因的启动子与GUS基因融合来分析水稻此基因的表达部位,是一种简便和有效方法.     

水稻ADP-葡萄糖焦磷酸化酶小亚基Ⅰ基因的启动子分析

水稻(Oryaz sativa L.)基因组中的ADP-葡萄糖焦磷酸化酶小亚基(ADP-Glucose pyrophosphorylase smallsubunit,OsAgpS)由两个基因编码,即OsAgpS1和OsAgpS2.其中OsAgpS1基因产生两个转录本OsAgpS1a和OsAgpS1b,区别在第一个外显子的位置不同.通过RT-PCR方法分析了两个转录本在水稻组织和胚乳不同发育时期的表达特性;同时通过报告基因GUS检测了两个转录本上游转录调节区DNA片段的转录启动特性.结果表明,两个启动了与其下游转录本的表达模式完全一致,即OsAgpS1a转录本和OsAgpS1a 上游启动子控制的GUS基因主要在胚乳中高水平表达,在叶片中有很低水平的表达;而OsAgpS1b转录本和OsAgpS1b上游启动子控制的GUS基因主要在叶片和胚乳发育早期低水平表达.这说明OsAgpS1基因产生的两个转录本是由不同的启动子控制转录的,OsAgpS1a上游启动了可以作为胚乳表达用启动子.     

水稻sbe1启动子驱动的反义sbe-GUS融合基因在转基因水稻中的表达

为研究水稻基因启动子对外源基因在转基因水稻中表达的影响,构建了由sbe1启动子引导的反义sbe-GUS融合基因。经农杆菌介导,将不同的融合基因导入水稻中,定量测定转基因水稻植株不同组织中的GUS酶活力。结果表明,sbe1启动子可驱动反义sbe-GUS融合基因在转基因水稻植株的胚乳中高效表达,而在颖壳、胚和茎叶等组织中的表达活性较弱。证实sbe1启动子在驱动外源基因的表达上表现有明显的组织特异性。     

水稻OsERF96应答病原菌的表达及启动子的功能分析

前人研究发现水稻Os ERF96(ethylene responsive factor 96)可应答白叶枯病病原菌的侵染,但其功能及表达调控机制仍不清楚,本研究进一步分析了该基因在水稻应答稻瘟病病原菌侵染及外源激素(SA和Me JA)处理下的转录情况,并分析了其启动子的诱导表达活性。结果表明:相对于对照组,Os ERF96在接种稻瘟病后1~4 d表达量显著上调,以第1天最高,此后逐渐下降,外源SA处理后Os ERF96表达量持续上调;利用Os ERF96启动子驱动GUS的转基因株系分析了Os ERF96启动子的诱导活性,结果表明GUS在根、茎和叶均有不同程度组成型表达,稻瘟病菌接种后4~7 d GUS活性持续升高。GUS活性定量表明,稻瘟病菌和SA处理条件下均出现了升高。综上所述,Os ERF96可应答白叶枯病或稻瘟病病原菌的浸染,其启动子是一个对病原菌侵染产生应答的诱导性启动子。     

水稻rbcS启动子控制的外源基因在转基因水稻中的特异性表达

为将不同启动子用于转基因水稻的研究,从武运粳8号水稻中克隆了Rubisco小亚基基因(rbcS)的5'上游调控区,构建了由rbcS启动子引导的GUS融合基因,并经农杆菌介导导入到水稻中.对转基因水稻植株中GUS活性的定性与定量测定结果表明,rbcS启动子可驱动GUS报告基因在转基因水稻植株叶片和叶鞘内的叶肉细胞中特异性高效表达,而在茎、根和种子等器官中不表达或表达活性极弱,表现出明显的组织与细胞特异性.结果还表明,光诱导处理可明显提高rbcS启动子启动的外源基因的表达量.     

Expression pattern and activity of six glutelin gene promoters in transgenic rice

The shortage of strong endosperm-specific expression promoters for driving the expression of recombinant protein genes in cereal endosperm is a major limitation in obtaining the required level and pattern of expression. Six promoters of seed storage glutelin genes (GluA-1, GluA-2, GluA-3, GluB-3, GluB-5, and GluC) were isolated from rice (Oryza sativa L.) genomic DNA by PCR. Their spatial and temporal expression patterns and expression potential in stable transgenic rice plants were examined with beta-glucuronidase (GUS) used as a reporter gene. All the promoters showed the expected spatial expression within the endosperm. The GluA-1, GluA-2, and GluA-3 promoters directed GUS expression mainly in the outer portion (peripheral region) of the endosperm. The GluB-5 and GluC promoters directed GUS expression in the whole endosperm, with the latter expressed almost evenly throughout the whole endosperm, a feature different from that of other rice glutelin gene promoters. The GluB-3 promoter directed GUS expression solely in aleurone and subaleurone layers. Promoter activities examined during seed maturation showed that the GluC promoter had much higher activity than the other promoters. These promoters are ideal candidates for achieving gene expression for multiple purposes in monocot endosperm but avoid promoter homology-based gene silencing. The GluC promoter did not contain the endosperm specificity-determining motifs GCN4, AACA, and the prolamin-box, which suggests the existence of additional regulatory mechanism in determining endosperm specificity.     

Promoters of Rice Seed Storage Protein Genes Direct Endosperm-Specific Gene Expression in Transgenic Rice

The promoters of genes encoding rice seed storage proteins (glutelin,prolamin, globulin and albumin) were analyzed for their abilityto direct rß-gIucuronidase (GUS) gene expression intransgenic rice plants. All promoters tested could direct endosperm-specificexpression of the GUS reporter gene irrespective of variableactivities and patterns in the endosperm. (Received February 27, 1998; Accepted May 16, 1998)     

Tissue-specific expression in transgenic maize of four endosperm promoters from maize and rice

The tissue-specific, developmental, and genetic control of four endosperm-active genes was studied via expression of GUS reporter genes in transgenic maize plants. The transgenes included promoters from the maize granule-bound starch synthase (Waxy) gene (zmGBS), a maize 27 kDa zein gene (zmZ27), a rice small subunit ADP-glucose pyrophosphorylase gene (osAGP) and the rice glutelin 1 gene (osGT1). Most plants had a transgene expression profile similar to that of the endogenous gene: expression in the pollen and endosperm for the zmGBS transgene, and endosperm only for the others. Histological analysis indicated expression initiated at the periphery of the endosperm for zmGBS, zmZ27 and osGT1, while osAGP transgene activity tended to start in the lower portion of the seed. Transgene expression at the RNA level was proportional to GUS activity, and did not influence endogenous gene expression. Genetic analysis showed that there was a positive dosage response with most lines. Activity of the zmGBS transgene was threefold higher in a low starch (shrunken2) genetic background. This effect was not seen with zmZ27 or osGT1 transgenes. The expression of the transgenes is discussed relative to the known behaviour of the endogenous genes, and the developmental programme of the maize endosperm     

Evaluation of tissue specificity and expression strength of rice seed component gene promoters in transgenic rice

Using stable transgenic rice plants, the promoters of 15 genes expressed in rice seed were analysed for their spatial and temporal expression pattern and their potential to promote the expression of recombinant proteins in seeds. The 15 genes included 10 seed storage protein genes and five genes for enzymes involved in carbohydrate and nitrogen metabolism. The promoters for the glutelins and the 13 kDa and 16 kDa prolamins directed endosperm-specific expression, especially in the outer portion (peripheral region) of the endosperm, whilst the embryo globulin and 18 kDa oleosin promoters directed expression in the embryo and aleurone layer. Fusion of the GUS gene to the 26 kDa globulin promoter resulted in expression in the inner starchy endosperm tissue. It should be noted that the 10 kDa prolamin gene was the only one tested that required both the 5' and 3' flanking regions for intrinsic endosperm-specific expression. The promoters from the pyruvate orthophosphate dikinase (PPDK) and ADP-glucose pyrophosphorylase (AGPase) small subunit genes were active not only in the seed, but also in the phloem of vegetative tissues. Within the seed, the expression from these two promoters differed in that the PPDK gene was only expressed in the endosperm, whereas the AGPase small subunit gene was expressed throughout the seed. The GUS reporter gene fused to the alanine aminotransferase (AlaAT) promoter was expressed in the inner portion of the starchy endosperm, whilst the starch branching enzyme (SBE1) and the glutamate synthase (GOGAT) genes were mainly expressed in the scutellum (between the endosperm and embryo). When promoter activities were examined during seed maturation, the glutelin GluB-4, 26 kDa globulin and 10 kDa and 16 kDa prolamin promoters exhibited much higher activities than the others. The seed promoters analysed here exhibited a wide variety of activities and expression patterns, thus providing many choices suitable for various applications in plant biotechnology.     

OsRRM, a Spen-like rice gene expressed specifically in the endosperm

We used the promoter trap technique to identify a rice plant, named 107^#, in which the β-glucuronidase （GUS） reporter gene was expressed specifically in the endosperm. A single copy of the T-DNA was inserted into the plant genome, and a candidate gene OsRRM was identified by the insertion. The OsRRM promoter directed GUS expression specifically in rice endosperm, analogous to the GUS expression pattern observed in 107^#. OsRRMis a single-copy gene in rice and encodes a nuclear protein containing 1 005 amino-acid residues with two RNA recognition motifs and one Spen paralog and ortholog C-terminal domain. Westem blot analysis confirmed that the OsRRM protein was specifically expressed in rice endosperm. Ectopic expression of OsRRM in transgenic plants led to abnormalities, such as short stature, retarded growth and low fructification rates. Our data, in conjunction with the reported function of Spen genes, implicated OsRRM in the regulation of cell development in rice endosperm.